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MBC in Press, published online ahead of print April 2, 2004
Mol. Biol. Cell 10.1091/mbc.E03-11-0844

A more recent version of this article appeared on June 1, 2004
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Submitted on November 25, 2003
Revised on March 13, 2004
Accepted on March 17, 2004

Diacylglycerol dependent binding recruits PKC{theta} and RasGRP1 C1 domains to specific subcellular localizations in living T lymphocytes

Silvia Carrasco1 and Isabel Merida1*

1 Department of Immunology and Oncology, National Center for Biotechnology, Consejo Superior de Investigaciones Científicas, Campus de Cantoblanco, E-28049 Madrid Spain

* Corresponding author. E-mail address: imerida{at}cnb.uam.es.

Diacylglycerol (DAG) signaling relies on the presence of conserved domain 1 (C1) in its target proteins. Phospholipase C-dependent generation of DAG following T cell receptor triggering is essential for the correct immune response onset. Accordingly, two C1-containing proteins expressed in T lymphocytes, Ras guanyl nucleotide-releasing protein1 (RasGRP1) and protein kinase C{theta} (PKC{theta}), were shown to be fundamental for T cell activation and proliferation. While containing the same regulatory domain, they are proposed to relocate to distinct subcellular locations in response to TCR triggering. Here we studied intracellular localization of RasGRP1 and PKC{theta} C1 domains in living Jurkat T cells. The results demonstrate that, in the absence of significant primary sequence differences, the C1 domains of these proteins show specific localization within the cell and distinct responses to pharmacological stimulation and T cell receptor triggering. These differences help explain the divergent localization and distinct functional roles of the full-length proteins, which contains them. The properties of these DAG-binding modules allow their characterization as functional markers that discriminate between DAG pools. Finally, we show that by binding to different diacylglycerol forms, overexpression of distinct C1 modules can attenuate DAG-dependent signals originating from the plasma or internal membranes. This is shown by analizing the contribution of these two lipid pools to PLC-dependent Ras activation in response to T cell receptor triggering.




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